Evaluation of E1B-mutant Replicating Adenoviruses for Cancer Gene Therapy / Journal of the Korean Cancer Association, 대한암학회지
Cancer Research and Treatment
; : 500-511, 2001.
Article
em Ko
| WPRIM
| ID: wpr-120298
Biblioteca responsável:
WPRO
ABSTRACT
PURPOSE: Gene-attenuated replication-competent adenoviruses are emerging as a promising new modality for the treatment of cancer. In an effort to continually improve upon cancer gene therapy, we have modified gene- attenuated replication-competent adenoviruses so as to cause them to replicate efficiently and lyse the infected cancer cells more effectively. MATERIALS AND METHODS: We modified the E1 region of the adenovirus (Ad) systematically, generating Ad-deltaE1B19, Ad-deltaE1B55, Ad-deltaE1B19/55, and Ad-WT. The cytopathic effects (CPE) and viral replication of these four gene modified adenoviruses were compared, and the morphology and DNA fragmentation of the infected cells was evaluated. RESULTS: Among the constructed adenoviruses, E1B 19kD-inactivated adenovirus (Ad-deltaE1B19) was the most potent, inducing the largest-sized plaques and markedCPE. Moreover, cells infected with Ad-deltaE1B19 showed complete cell lysis with disintegrated cellular structure whereas cells infected with Ad-WT maintained intact cellular and nuclear membrane with properly structured organelles. TUNEL assay was also used to monitor DNA integrity, and a more profound induction of apoptosis was observed in the Ad-deltaE1B19 infected cells in comparison to wild type adenovirus infected cells. CONCLUSION: We demonstrate that the inactivation of the E1B19kD gene in a replicating adenovirus leads to increased CPE, rapid viral release, improved cell-to-cell viral spread and increased induction of apoptosis.
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Texto completo:
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Índice:
WPRIM
Assunto principal:
DNA
/
Organelas
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Adenoviridae
/
Apoptose
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Marcação In Situ das Extremidades Cortadas
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Estruturas Celulares
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Genes Neoplásicos
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Fragmentação do DNA
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Membrana Nuclear
Idioma:
Ko
Revista:
Cancer Research and Treatment
Ano de publicação:
2001
Tipo de documento:
Article